Thermophilic Organisms For Conversion of Lignocellulosic Biomass To Ethanol

ABSTRACT

Mutant thermophilic organisms that consume a variety of biomass derived substrates are disclosed herein. Strains of  Thermoanaerobacterium saccharolyticum  with acetate kinase and phosphotransacetylase expression eliminated are disclosed herein. Further, strain ALK1 has been engineered by site directed homologous recombination to knockout both acetic acid and lactic acid production. Continuous culture involving a substrate concentration challenge lead to evolution of ALK1, and formation of a more robust strain designated ALK2. Both organisms produce near theoretical ethanol yields without expressing pyruvate decarboxylase

RELATED APPLICATIONS

This application claims priority to U.S. application No. 60/731,674, filed Oct. 31, 2005, and to U.S. application No. 60/796,380, filed May 1, 2006, each of which is incorporated herein by reference.

GOVERNMENT INTERESTS

The United States Government may have certain rights in the present invention as research relevant to its development was funded by National Institute of Standards and Technology (NIST) contract number 60NANB1D0064.

BACKGROUND

1. Field of the Invention

The present invention pertains to the field of biomass processing to produce ethanol. In particular, novel thermophilic organisms that consume a variety of biomass derived substrates and produce ethanol in high yield are disclosed, as well as processes for the production and use of the organisms.

2. Description of the Related Art

Biomass represents an inexpensive and readily available cellulolytic substrate from which sugars may be produced. These sugars may be used alone or fermented to produce alcohols and other products. Among bioconversion products, interest in ethanol is high because it may be used as a renewable domestic fuel.

Significant research has been performed in the areas of reactor design, pretreatment protocols and separation technologies, so that bioconversion processes are becoming economically competitive with petroleum fuel technologies. However, it is estimated that the largest cost savings may be obtained when two or more process steps are combined. For example, simultaneous saccharification and fermentation (SSF) and simultaneous saccharification and co-fermentation (SSCF) processes combine an enzymatic saccharification step with fermentation in a single reactor or continuous process apparatus. In addition to savings associated with shorter reaction times and reduced capital costs, co-fermentation processes may also provide improved product yields because certain compounds that would otherwise accrue at levels that inhibit metabolysis or hydrolysis are consumed by the co-fermenting organisms. In one such example, β-glucosidase ceases to hydrolyze cellobiose in the presence of glucose and, in turn, the build-up of cellobiose impedes cellulose degradation. An SSCF process involving co-fermentation of cellulose and hemicellulose hydrolysis products may alleviate this problem by converting glucose into one or more products that do not inhibit the hydrolytic activity of β-glucosidase.

Consolidated bioprocessing (CBP) involves four biologically-mediated events: (1) enzyme production, (2) substrate hydrolysis, (3) hexose fermentation and (4) pentose fermentation. These events may be performed in a single step. This strategy requires a microorganism that utilizes cellulose and hemicellulose. Development of CBP organisms could potentially result in very large cost reductions as compared to the more conventional approach of producing saccharolytic enzymes in a dedicated process step. CBP processes that utilize more than one organism to accomplish the four biologically-mediated events are referred to as consolidated bioprocessing co-culture fermentations.

Some bacteria have the ability to convert pentose sugars into hexose sugars, and to ferment the hexose sugars into a mixture of organic acids and other products by glycolysis. The glycolytic pathway begins with conversion of a six-carbon glucose molecule into two three-carbon molecules of pyruvate. Pyruvate may then be converted to lactate by the action of lactate dehydrogenase (“ldh”), or to acetyl coenzyme A (“acetyl-CoA”) by the action of pyruvate dehydrogenase or pyruvate-ferredoxin oxidoreductase. Acetyl-CoA is further converted to acetate by phosphotransacetylase and acetate kinase, or reduced to ethanol by acetaldehyde dehydrogenase (“AcDH”) and alcohol dehydrogenase (“adh”). Overall, the performance of ethanol-producing organisms is compromised by production of organic products other than ethanol, and particularly by ldh-mediated conversion of pyruvate to lactate, and by conversion of acetyl-CoA to acetate by phosphotransacetylase and acetate kinase.

Metabolic engineering of bacteria has recently resulted in the creation of a knockout of lactate dehydrogenase in the thermophilic, anaerobic, Gram-positive bacterium T. saccharolyticum. See, Desai, S. G.; Guerinot, M. L.; Lynd, L. R. “Cloning of L-lactate dehydrogenase and elimination of lactic acid production via gene knockout in Thermoanaerobacterium saccharolyticum JW/SL-YS485” Appl. Microbiol. Biotechnol. 65: 600-605, 2004.

Although the knockout of ldh constitutes an advance in the art, it is problematic for some uses of this organism in that this strain of T. saccharolyticum continues to make organic acid—in particular, acetic acid.

SUMMARY

The present instumentalities advance the art and overcome the problems outlined above by providing thermophilic, anaerobic bacteria that consume a variety of biomass derived substrates and produce ethanol in near theoretical yields. Methods for producing ethanol using the organisms are also disclosed.

The instrumentalities reported herein result in the knockout of various genes either singly or in combination, where such genes in the native organism would otherwise result in the formation of organic acids. For example, there may be knockouts of: (a) acetate kinase and/or phosphotransacetylase and (b) lactate dehydrogenase (ldh), acetate kinase (ack) and phosphotransacetylase (pta) in T. saccharolyticum JW/SL-YS485. Although the results reported herein are for T. saccharolyticum, the methods and materials also apply to other members of the Thermoanaerobacter genus including Thermoanaerobacterium thermosulfurigenes, Thermoanaerobacterium aotearoense, Thermoanaerobacterium polysaccharolyticum, Thermoanaerobacterium zeae, Thermoanaerobacterium thermosaccharolyticum, and Thermoanaerobacterium xylanolyticum. The methods and materials are useful generally in the field of metabolically engineered, thermophilic, Gram-positive bacteria.

In one embodiment, an isolated organism, which does not express pyruvate decarboxylase, ferments a cellulolytic substrate to produce ethanol in a concentration that is at least 90% of a theoretical yield.

In one embodiment, a Gram-positive bacterium, that in a native state contains at least one gene which confers upon the Gram-positive bacterium an ability to produce acetic acid as a fermentation product, is transformed to eliminate expression of the at least one gene. The bacterium may be a Thermoanaerobacter, such as Thermoanaerobacterium saccharolyticum. The gene which confers upon the Gram-positive bacterium an ability to produce acetic acid as a fermentation product may code for expression of acetate kinase and/or phosphotransacetylase.

In another embodiment, the Gram-positive bacterium may be further transformed to eliminate expression of one or more genes that confer upon the Gram-positive bacterium the ability to produce lactic acid as a fermentation product. For example, the gene that confers the ability to produce lactic acid may be lactate dehydrogenase.

In one embodiment, a method for producing ethanol includes transforming a native organism to produce a Gram-positive bacterium that has been transformed to eliminate expression of all genes that confer upon the Gram-positive bacterium the ability to produce organic acids as fermentation products, to produce a transformed bacterial host, and culturing the transformed bacterial host in medium that contains a substrate including a material selected from the group consisting of glucose, xylose, cellobiose, sucrose, xylan, starch, and combinations thereof under suitable conditions for a period of time sufficient to allow saccharification and fermentation of the substrate.

In one embodiment, a biologically pure culture of a microorganism designated ALK1 and deposited with the ATCC under Patent Deposit Designation No. PTA-7206 is described.

In one embodiment an isolated polynucleotide comprises (a) a sequence of SEQ ID NO: 10, or (b) a sequence of SEQ ID NO: 9 and SEQ ID NO: 10, or (c) a sequence having at least about 90% sequence identity with the sequence of (a) or (b). A vector comprising the isolated polynucleotide of (a), (b), or (c) is described, as well as a host cell genetically engineered to express a compliment of the polynucleotide of (a), (b), or (c). In another embodiment, an isolated polynucleotide comprises a sequence having at least about 95% sequence identity with-the sequence of (a) or (b).

In one embodiment, a method of producing ethanol includes culturing a mutant bacterium expressing a compliment of the isolated polynucleotide of (a), (b), or (c) in medium containing a substrate selected from the group consisting of glucose, xylose, cellobiose, sucrose, xylan, starch, and combinations thereof under suitable conditions for a period of time sufficient to allow fermentation of the substrate to ethanol.

BRIEF DESCRIPTION OF THE DRAWINGS

FIG. 1 shows reactions of the glycolytic pathway.

FIG. 2 shows hydrogen production in wild-type T. saccharolyticum compared to various knockout strains of T. saccharolyticum.

FIG. 3 shows a comparison of experimental and expected polynucleotide sequences for the ldh region of the suicide vector pSGD9 (SEQ ID NO: 9) integrated into the genome of T. saccharolyticum.

FIG. 4 shows a comparison of experimental and expected polynucleotide sequences for the pta/ack region of the suicide vector pSGD8-Erm (SEQ ID NO: 10) integrated into the genome of T. saccharolyticum.

FIGS. 5-7 show high-performance liquid chromotography (HPLC) traces of a fermentation broth at various time intervals during growth of ALK1.

FIG. 8 shows xylose, organic acid and ethanol concentrations during fermentation by strain ALK1.

FIG. 9 shows xylose, organic acid and ethanol concentrations during fermentation by wild-type T. saccharolyticum.

FIG. 10 shows xylose, organic acid and ethanol concentrations during a continuous culture challenge of ALK1.

FIG. 11 shows xylose, organic acid and ethanol concentrations during fermentation by strain ALK2.

DETAILED DESCRIPTION

There will now be shown and described methods for engineering and utilizing thermophilic, anaerobic, Gram-positive bacteria in the conversion of biomass to ethanol.

As used herein, an organism is in “a native state” if it is has not been genetically engineered or otherwise manipulated by the hand of man in a manner that intentionally alters the genetic and/or phenotypic constitution of the organism. For example, wild-type organisms may be considered to be in a native state.

Complete elimination of organic acid production from a T. saccharolyticum in a native state was achieved using two site-directed DNA homologous recombination events. The mutant strain, Thermoanaerobacterium saccharolyticum JW/SL-YS485 ALK1 (“ALK1”) produces near theoretical amounts of ethanol at low substrate feedings in batch culture with a temperature in a range of about 30-66° C. and a pH in a range of about 3.85-6.5. In one embodiment, ethanol yield is at least about 90% of the theoretical maximum. ALK1, and its decendents, have the potential to contribute significant savings in the lignocellulosic biomass to ethanol conversion due to its growth conditions, which are substantially optimal for cellulase activity in a simultaneous saccharification and co-fermentation (SSCF) process. For example, optimal cellulase activity parameters include a pH between 4-5 and temperature between 40-50° C. Additionally, it is unnecessary to adjust the pH of the fermentation broth when knockout organisms, which lack the ability to produce organic acids, are used. ALK1, and similar organisms, may also be suitable for a consolidated bioprocessing co-culture fermentation where the knockout organism would convert pentoses to ethanol, and cellulose would be degraded by a cellulolytic organism such as C. thermocellum.

Operating either an SSCF or CBP process at thermophilic temperatures offers several important benefits over conventional mesophilic fermentation temperatures of 30-37° C. In particular, costs for a process step dedicated to cellulase production are substantially reduced (e.g., 2-fold or more) for thermophilic SSCF and are eliminated for CBP. Costs associated with fermentor cooling and also heat exchange before and after fermentation are also expected to be reduced for both thermophilic SSCF and CBP. Finally, processes featuring thermophilic biocatalysts may be less susceptible to microbial contamination as compared to processes featuring conventional mesophilic biocatalysts.

In contrast to known “homoethanol-fermenting” microorganisms, such as naturally-occurring Saccharomyces cerevisiae and Zymomonas mobilis, and recombinant strains of Escherchia coli and Klebsiella oxytoca, the presently disclosed organisms do not depend on conversion of pyruvate to acetaldehyde via the action of pyruvate decarboxylase (FIGS. 1, 9). In fact, bacteria belonging to the Thermoanaerobacter genus do not express pyruvate decarboxylase in the native state. From the reactions of the glycolytic pathway shown in FIG. 1, it can be observed that pyruvate may be metabolized to acetyl-CoA, carbon dioxide, and reduced ferredoxin by the enzyme pyruvate-ferredoxin oxidoreductase, 2. However, in order to produce ethanol as the only fermentation product, the electrons carried by reduced ferredoxin must all be transferred to NAD via NAD:ferredoxin oxidoreductase, 3, to form NADH. NADH is subsequently oxidized back to NAD in the course of the two-step reduction of acetyl-CoA to ethanol by acetaldehyde dehydrogenase, 7, and alcohol dehydrogenase, 8. Evidence of the efficient utilization of NADH may be observed in FIG. 2 as a decrease in production of H₂ by both the acetate knockout organism, which is unable to express ack and pta, and the double knockout organism (ALK1), which is unable to express ack, pta and ldh. These organisms provide the first demonstration of stoichiometric electron transfer from reduced ferredoxin to NAD, and subsequently to ethanol.

The above-described pathway, which produces stoichiometric ethanol yields in organisms that do not possess the ability to express PDC, is in contrast to the pathway employed in all previously-described homoethanol-fermenting strains. Previously-described strains utilize endogenous pyruvate decarboxylase (PDC), or are engineered to express exogenous PDC. Since expression of PDC is rare in the microbial world, the ability to redirect electron flow by virtue of modifications to carbon flow has broad implications. For example, this approach could be used to produce high ethanol yields in strains other than T. saccharolyticum and/or to produce solvents other than ethanol. In particular, Gram-positive bacteria, such as members of the Thermoanaerober genus; Clostridium thermocellum and other thermophilic and mesophilic Clostridia; thermophilic and mesophilic Bacillus species; Gram-negative bacteria, such as Escherichia coli and Klebsiella oxytoca; Fibrobacter succinogenes and other Fibrobacter species; Thermoga neopolitana and other Thermotoga species; and anaerobic fungi including Neocallimatix and Piromyces species lack the ability to express PDC, and may benefit from the disclosed instrumentalities.

It will be appreciated that the lignocellulosic material may be any feedstock that contains one or more of glucose, xylose, mannose, arabinose, galactose, fructose, cellobiose, sucrose, maltose, xylan, mannan and starch. In various embodiments, the lignocellulosic biomass comprises wood, corn stover, sawdust, bark, leaves, agricultural and forestry residues, grasses such as switchgrass, ruminant digestion products, municipal wastes, paper mill effluent, newspaper, cardboard, or combinations thereof.

EXAMPLE 1 Production of the ALK1 Strain Materials and Methods

Thermoanaerobacterium saccharolyticum strain JW/SL-YS485 (DSM 8691) is a thermophilic, anaerobic bacteria isolated from the West Thumb Basin in Yellowstone National Park, Wyo. (Lui, S. Y; Gherardini, F. C.; Matuschek, M.; Bahl, H.; Wiegel, J. “Cloning, sequencing, and expression of the gene encoding a large S-layer-associated endoxylanase from Thermoanaerobacterium sp strain JW/SL-YS485 in Escherichia coli” J. Bacteriol. 178: 1539-1547, 1996; Mai, V.; Wiegel, J. “Advances in development of a genetic system for Thermoanaerobacterium spp: Expression of genes encoding hydrolytic enzymes, development of a second shuttle vector, and integration of genes into the chromosome” Appl. Environ. Microbiol. 66: 4817-4821, 2000). It grows in a temperature range of 30-66° C. and in a pH range of 3.85-6.5. It consumes a variety of biomass derived substrates including the monosaccharides glucose and xylose, the disaccharides cellobiose and sucrose, and the polysaccharides xylan and starch, but not cellulose. The organism produces ethanol as well as the organic acids lactic acid and acetic acid as primary fermentation products.

Cloning and Sequencing

The lactate dehydrogenase (L-ldh), phosphotransacetylase (pta), and acetate kinase (ack) genes were identified and sequenced using standard techniques, as reported previously for L-ldh (Desai, 2004). Degenerate primers were made using the CODE-HOP algorithm (Rose, T.; Schultz, E.; Henikoff, J.; Pietrokovski, S.; McCallum, C.; Henikoff, S. “Consensus-degenerate hybrid oligonucleotide primers for amplification of distantly-related sequences” Nucleic Acids Research, 26(7):1628-1635, 1 Apr. 1998) and PCR reactions were performed to obtain the DNA sequence between conserved regions. The gene fragments outside of the conserved regions were sequenced directly from genomic DNA using ThermoFidelase (Fidelity Systems, Gaithersburg, Md.) enzyme with BigDye Terminator kit v3.1 (ABI, Foster City Calif.).

Construction of Suicide Vectors

Acetate kinase and phosphotransacetylase knockout vector, pSGD9

Standard cloning techniques were followed (Sambrook). The 6.2 kb suicide vector pSGD9 was based on pBLUESCRIPT II SK (+) (Stratagene) using a design approach similar to that reported earlier (Desai, 2004; Mai, 2000). Gene fragments of the pta/ack sequence, pta-up (˜1.2 kb) and ack-down (˜0.6 kb), were amplified from genomic DNA using primer pairs SEQ ID NOS: 1-2, and SEQ ID NOS: 3-4. PCR amplification was performed with pfu DNA polymerase and the fragments were extracted from a 1% electrophoresis gel. Fragments pta-up and ack-down were then A-tailed with Taq polymerase and cloned into TOPO pCR2.1 (Invitrogen, Carlsbad, Calif.). A 1.5 kb fragment containing the kanamycin marker was obtained from a PstI/XbaI digest of pIKM1 and subcloned into pBLUESCRIPT II SK (+). TOPO containing pta-up was digested with XhoI/BsiHK4I and subcloned into XhoI/PstI digested pBLUESCRIPT II SK (+), upstream of the previously subcloned kanamycin marker. TOPO containing ack-down was digested with XbaI/SphI and subcloned into pUC19 (Invitrogen). XbaI/AƒIII fragment containing ack-down was digested and subcloned downstream of the kanamycin marker to obtain the. final construct pSGD9.

Lactate Dehydrogenase Knockout Vector with Erythromycin Resistance, pSGD8-Erm

The 5.5 kb suicide vector pSGD8-Erm was based on the plasmid pSGD8 as produced by Desai et al. 2004. In place of the aph kanamycin antibiotic marker, a fusion gene based on the aph promoter from the plasmid pIKM1 and the adenine methylase gene conferring erythromycin resistance from the plasmid pCTC1 (Klapatch, T. R.; Guerinot, M. L.; Lynd, L. R. “Electrotransformation of Clostridium thermosaccharolyticum” J. Ind. Microbiol. 16(6): 342-7, June 1996) were used for selection. PCR gene fragments were created using pfu polymerase (Stategene) and the primers SEQ ID NOS: 5-6 for the aph promoter and SEQ ID NOS: 7-8 for the adenine methylase open reading frame. Fragments were digested with XbaI/BamH1 (aph fragment) and BamHI/EcoRI (adenine methylase) and ligated into the multiple cloning site of pIKM1. This fusion gene was then excised with BseRI/EcoRI and ligated into similarly digested pSGD8.

Transformation of T. saccharolyticum

Transformation of T saccharolyticum was performed interchangeably with two methods, the first as previously described (Mai, V.; Lorenz, W.; Weigel, J. “Transformation of Thermoanaerobacterium sp. strain JW/SL-YS485 with plasmid PIKM1 conferring kanamycin resistance” FEMS Microbiol. Lett. 148: 163-167, 1997) and the second with several modifications following cell harvest and based on the method developed for Clostridium thermocellum (Tyurin, M. V.; Desai, S. G.; Lynd, L. R. “Electrotransformation of Clostridium thermocellum” Appl. Environ. Microbiol. 70(2): 883-890, 2004). Cells were grown overnight using pre-reduced medium DSMZ 122 in sterile disposable culture tubes inside an anaerobic chamber in an incubator maintained at 55° C. Thereafter, cells were sub-cultured with 4 μg/ml isonicotonic acid hydrazide (isoniacin), a cell wall weakening agent (Hermans, J.; Boschloo, J. G.; de Bont, J. A. M. “Transformation of M. aurum by electroporation: the use of glycine, lysozyme and isonicotinic acid hydrazide in enhancing transformation efficiency” FEMS Microbiol. Lett. 72, 221-224, 1990), added to the medium after the initial lag phase. Exponential phase cells were harvested and washed with pre-reduced cold sterile 200 mM cellobiose solution, and resuspended in the same solution and kept on ice. Extreme care was taken following the harvesting of cells to keep them cold (approximately 4° C.) at all times including the time during centrifugation.

Samples composed of 90 μl of the cell suspension and 2 to 6 μl of pSGD9 or pSGD8-Erm (1 to 3 μg) added just before pulse application, were placed into sterile 2 ml polypropylene microcentrifuge disposable tubes that served as electrotransformation cuvettes. A square-wave with pulse length set at 10 ms was applied using a custom-built pulse generator/titanium electrode system. A voltage threshold corresponding to the formation of electropores in a cell sample was evaluated as a non-linear current change when pulse voltage was linearly increased in 200V increments. A particular voltage that provided the best ratio of transformation yield versus cell viability rate at a given DNA concentration was used, which in this particular case was 25 kV/cm. Pulsed cells were initially diluted with 500 μl DSM 122 medium, held on ice for 10 minutes and then recovered at 55° C. for 4-6 hrs. Following recovery, cells transformed with pSGD9 were mixed with 2% agar medium containing kanamycin at 75 μg/ml and poured onto petri plates and incubated in anaerobic jars for 4 days. Cells transformed with pSGD8-Erm were allowed to recover at 48° C. for 4-6 hrs and were either plated in 2% agar medium at pH 6.0 containing erythromycin at 5 μg/ml or similar liquid media and incubated in anaerobic jars at 48° C. for 6 days. Either of the transformed cell lines may be used without further manipulation. However, an organism where elimination of expression of all genes that confer the ability to produce organic acids was obtained by performing a second (sequential) transformation. The second transformation was carried out as described above with the primary transformant substituted for the non-transformed cell suspension. The secondary transformant, ALK1, was grown on medium containing both kanamycin and erythromycin.

Sequencing of Knockout Regions

Sequencing of the site directed knockout regions was done by PCR from genomic DNA using Taq polymerase (New England Biolabs) and primers outside the regions of homologous overlap between the genome and the suicide vectors. Primers inside the PCR products were used for sequencing with the BigDye Terminator kit v3.1 (ABI, Foster City, CA). Regions were arranged using the CAP3 software program (Huang, X. “An improved sequence assembly program” Genomics 33: 21-31, 1996) and compared to the expected DNA sequence using the CLUSTAL W algorithm (Higgins, D. G.; Bleasby, A. J.; Fuchs, R. “CLUSTAL V: improved software for multiple sequence alignment” Computer Applications in the Biosciences (CABIOS), 8(2): 189-191, 1992). A high degree of homology (percent identity) existed between the experimentally compiled sequence and the expected sequence based on the known wild-type and suicide vector sequences (FIGS. 3 and 4).

“Identity” refers to a comparison between pairs of nucleic acid or amino acid molecules. Methods for determining sequence identity are known. See, for example, computer programs commonly employed for this purpose, such as the Gap program (Wisconsin Sequence Analysis Package, Version 8 for Unix, Genetics Computer Group, University Research Park, Madison Wis.), that uses the algorithm of Smith and Waterman, 1981, Adv. Appl. Math. 2: 482-489.

Verification of Mutant Strain

Genomic DNA from the mutant strain Thermoanaerobacterium saccharolyticum JW/SL-YS485 ALK1 (“ALK1”) showed the expected site-directed homologous recombination in the L-ldh and pta/ack loci through DNA sequencing. Both integration events were double integrations, which is a more genetically stable genotype.

EXAMPLE 2 Comparative Data Showing Production of Ethanol by ALK1 and Wild-Type T. Saccharolyticum

T. saccharolyticum was grown in partially defined MTC media containing 2.5 g/L Yeast Extract (Zhang, Y.; Lynd, L. R. “Quantification of cell and cellulase mass concentrations during anaerobic cellulose fermentation: development of an enzyme-linked immunosorbent assay-based method with application to Clostiridium thermocellum batch cultures” Anal. Chem. 75: 219-222, 2003). Glucose, xylose, acetate, lactate and ethanol were analyzed by HPLC on an Aminex 87H column (BioRad Laboratories, Hercules, Calif.) at 55° C. The mobile phase consisted of 5 mM sulfuric acid at a flow rate of 0.7 ml/min. Detection was via refractive index using a Waters 410 refractometer (Milford, Mass.). The minimum detection level for acetate was 1.0 mM. A standard trace containing 5 g/L xylose, 5 g/L lactic acid, 5 g/L acetic acid and 5 g/L ethanol is shown in FIG. 5.

Strain ALK1 produced only ethanol with up to 17 g/L xylose, or with 5 g/L xylose and 5 g/L glucose, with no organic acids or other products detected by HPLC. FIG. 6 shows the ALK1 strain fermentation at time 0 hours and FIG. 7 shows the same fermentation at 72 hours. Time course fermentation plots of strain ALK1 and wild-type on xylose media buffered with 8 g/L MES at an initial pH of 6.0, 55° C. and 100 rpm show that strain ALK1 is able to convert over 99% of xylose to ethanol (FIG. 8), while the wild-type under similar conditions becomes pH limited due to organic acid production and is unable to consume all the xylose present (FIG. 9). The wild-type organism yielded 0.15 mM ethanol, while ALK1 yielded 0.46 mM ethanol.

EXAMPLE 3 Evolution of ALK1

As shown in FIG. 10, a continuous culture in which feed substrate concentration was increased over time was utilized to challenge ALK1. FIG. 10 shows xylose, xylulose and ethanol concentrations during the continuous culture. After more than 1000 hours of exposure to this stress-evolution cycle, an improved strain, ALK2, was isolated from the fermentation broth. ALK2 was able to initiate growth at 50 g/L xylose in batch culture. FIG. 11 shows xylose, organic acid, optical density (OD) and ethanol concentrations during fermentation by strain ALK2.

Deposit of ALK1

ALK1 has been deposited with the American Type Culture Collection, Manassas, Va. 20110-2209. The deposit was made on Nov. 1, 2005 and received Patent Deposit Designation Number PTA-7206. This deposit was made in compliance with the Budapest Treaty requirements that the duration of the deposit should be for thirty (30) years from the date of deposit or for five (5) years after the last request for the deposit at the depository or for the enforceable life of a U.S. Patent that matures from this application, whichever is longer. ALK1 will be replenished should it become non-viable at the depository.

The description of the specific embodiments reveals general concepts that others can modify and/or adapt for various applications or uses that do not depart from the general concepts. Therefore, such adaptations and modifications should and are intended to be comprehended within the meaning and range of equivalents of the disclosed embodiments. It is to be understood that the phraseology or terminology employed herein is for the purpose of description and not limitation.

The foregoing examples may be suitably modified for use upon any Gram-positive bacterium, and especially members of the Thermoanaerobacter genus including Thermoanaerobacterium thermosulfurigenes, Thermoanaerobacterium aotearoense, Thermanaerobacterium polysaccharolyticwum, Thermoanaerobacterium zeae, Thermoanaerobacterium thermosaccharolyticum, and Thermoanaerobacterium xylanolyticum.

All references mentioned in this application are incorporated by reference to the same extent as though fully replicated herein. 

1. An isolated organism that ferments a cellulolytic substrate to produce ethanol in a concentration that is at least 90% of a theoretical yield, wherein the organism does not express pyruvate decarboxylase.
 2. A method for producing ethanol, said method comprising: transforming a native organism to produce the isolated organism of claim 1 to provide a transformed host; and culturing the transformed host in medium that contains a substrate including a material selected from the group consisting of glucose, xylose, mannose, arabinose, galactose, fructose, cellobiose, sucrose, maltose, xylan, mannan, starch, and combinations thereof under suitable conditions for a period of time sufficient to allow saccharification and fermentation of the substrate.
 3. A transformed organism comprising, a Gram-positive bacterium that in a native state contains at least one gene which confers upon the Gram-positive bacterium an ability to produce acetic acid as a fermentation product, the Gram-positive bacterium being transformed to eliminate expression of the at least one gene.
 4. The Gram-positive bacterium according to claim 3, wherein the Gram-positive bacterium is a member of the Thermoanaerobacter genus.
 5. The Gram-positive bacterium according to claim 3, wherein the Gram-positive bacterium is a Thermoanaerobacterium saccharolyticum.
 6. The Gram-positive bacterium according to claim 3, wherein the at least one gene codes for expression of acetate kinase.
 7. The Gram-positive bacterium according to claim 3, wherein the at least one gene codes for the expression of phosphotransacetylase.
 8. The Gram-positive bacterium according to claim 3, wherein the at least one gene includes a plurality of genes.
 9. The Gram-positive bacterium according to claim 8, wherein the plurality of genes code for expression of acetate kinase and phosphotransacetylase.
 10. The Gram-positive bacterium according to claim 9, further transformed to eliminate expression of one or more genes that confer upon the Gram-positive bacterium the ability to produce lactic acid as a fermentation product.
 11. The Gram-positive bacterium according to claim 3, further transformed to eliminate expression of one or more genes that confer upon the Gram-positive bacterium the ability to produce lactic acid as a fermentation product.
 12. The Gram-positive bacterium according to claim 11, wherein the at least one gene codes for the expression of lactate dehydrogenase.
 13. A method for producing ethanol, said method comprising: transforming a native organism to produce the Gram-positive bacterium of claim 11 to produce a transformed bacterial host; and culturing the transformed bacterial host in medium that contains a substrate including a material selected from the group consisting of glucose, xylose, mannose, arabinose, galactose, fructose, cellobiose, sucrose, maltose, xylan, mannan, starch, and combinations thereof under suitable conditions for a period of time sufficient to allow saccharification and fermentation of the substrate.
 14. The method according to claim 13, wherein said bacterial host is a Thermoanaerobacterium saccharolyticum.
 15. The method according to claim 13, wherein the genes code for the expression of lactate dehydrogenase, acetate kinase, and phosphotransacetylase.
 16. A biologically pure culture of a microorganism designated ALK1 and deposited under Patent Deposit Designation No. PTA-7206.
 17. An isolated polynucleotide comprising: (a) a sequence of SEQ ID NO: 10; (b) a sequence of SEQ ID NO: 9 and SEQ ID NO: 10; or (c) a sequence having at least about 90% sequence identity with the sequence of (a) or (b).
 18. The polynucleotide of claim 17, having about 95% sequence identity with the sequence of (a) or (b).
 19. A vector comprising the isolated polynucleotide of claim
 18. 20. A host cell genetically engineered to express a compliment of the polynucleotide of claim
 18. 21. The host cell of claim 20, wherein the host cell is a bacterial cell.
 22. A method of producing ethanol comprising the step of: culturing a mutant bacterium according to claim 21 in medium containing a substrate selected from the group consisting of glucose, xylose, mannose, arabinose, galactose, fructose, cellobiose, sucrose, maltose, xylan, mannan, starch, and combinations thereof under suitable conditions for a period of time sufficient to allow fermentation of the substrate to ethanol.
 23. The method of claim 22, wherein the mutant bacterium is Thermoanaerobacterium saccharolyticum.
 24. The method of claim 23, wherein the mutant bacterium is Thermoanaerobacterium saccharolyticum ALK1 (JW/SL-YS485 ALK1).
 25. A genetic construct comprising SEQ ID NO: 10 operably connected to a promoter expressible in a bacterium.
 26. A recombinant bacterium comprising the genetic construct of claim
 25. 27. The recombinant bacterium of claim 26, wherein said bacterium is Thermoanaerobacterium saccharolyticum. 